Leaf and Flower Extracts from the Dwarf Elder (Sambucus ebulus): Toxicity and Repellence against Cosmopolitan Mosquito-Borne Diseases Vectors

Simple Summary There has been no scientific evidence of the bioactivity of Sambucus ebulus (Adoxaceae) extracts against insects. Therefore, we extracted and chemically characterized the leaves and flowers of S. ebulus in methanol and water. The two crude extracts and some of the phenolic compounds and amino acids isolated were tested as larvicides against two cosmopolitan mosquito species, namely the Asian tiger mosquito (Aedes albopictus) and the common house mosquito (Culex pipiens). To better understand their mode of action, we evaluated the in vitro acetylcholinesterase inhibitor effect of crude extracts on the two mosquito larvae by means of a colorimetric method. In addition, the ovideterrent effect of the crude extracts against Ae. albopictus females ovipositing in the open field was evaluated. Abstract As there has been no scientific evidence of the bioactivity of Sambucus ebulus (Adoxaceae) extracts against insects, we chemically characterized S. ebulus leaves and flowers extracted in methanol and water. The crude extracts, phenolic compounds, and amino acids isolated were tested as larvicides against the fourth-instar larvae of Aedes albopictus and Culex pipiens (Diptera: Culicidae). To understand their mode of action, we evaluated the in vitro acetylcholinesterase (AChE) inhibitor effect of the crude extracts on the two mosquito larvae through a colorimetric method. Furthermore, the deterrent effect of the crude extracts against ovipositing Ae. albopictus females was assessed in the open field. Twelve phenylpropanoids and fourteen amino acids were detected in the extracts, with a prevalence of hydroxycinnamic acids and nonaromatic amino acids. The most toxic compound to Ae. albopictus larvae after 24 h was gallic acid, followed by the crude S. ebulus leaf extract; on Cx. pipiens, it was the crude flower extract. The AChE test showed higher inhibition on both mosquito species exerted by the leaf extract if compared to the flower extract, and it also deterred oviposition by Ae. albopictus females starting from the third day. The results indicated that vegetal extracts could effectively help in the integrated vector management of mosquitoes.


Introduction
Sambucus ebulus L. (Adoxaceae), known as the dwarf elder for its moderate height (1-1.5 m), is an herbaceous perennial plant characterized by opposite, pinnate leaves and corymb inflorescences of white or pinkish flowers [1].It is widespread in woods, uncultivated lands, ditches, damp places, and along country lanes from central and southern Cx.pipiens fourth-instar larvae under laboratory conditions.To better understand their mode of action, we evaluated the in vitro acetylcholinesterase (AChE) inhibitor effect of the crude extracts on the two mosquito larvae through a colorimetric method.Furthermore, the deterrent effect of the crude extracts against ovipositing Ae. albopictus females was assessed in the open field.

Sambucus ebulus Vegetal Material
Sambucus ebulus leaves and flowers were harvested along the riverbanks of the Arno River in Pisa (Tuscany, Italy), where the plant grows luxuriantly, during July 2021.Plant material was frozen immediately in liquid nitrogen and stored at −80 • C after harvest.
The diagram of the experimental design is given in Figure 1.
possible usefulness of the dwarf elder in the control of mosquito populations.Therefore, we extracted and chemically characterized (through chromatographic techniques) leaves and flowers of S. ebulus components (i.e., phenylpropanoids (in methanol) and amino acids (in water)).The two crude extracts and some of the phenolic compounds (chlorogenic, gallic, hydroxybenzoic, and rosmarinic acids) and amino acids (arginine, aspartate, glutamic acid, histidine, serine, and threonine) isolated were tested as toxic agents for Ae.albopictus and Cx.pipiens fourth-instar larvae under laboratory conditions.To better understand their mode of action, we evaluated the in vitro acetylcholinesterase (AChE) inhibitor effect of the crude extracts on the two mosquito larvae through a colorimetric method.Furthermore, the deterrent effect of the crude extracts against ovipositing Ae. albopictus females was assessed in the open field.

Sambucus ebulus Vegetal Material
Sambucus ebulus leaves and flowers were harvested along the riverbanks of the Arno River in Pisa (Tuscany, Italy), where the plant grows luxuriantly, during July 2021.Plant material was frozen immediately in liquid nitrogen and stored at −80 °C after harvest.
The diagram of the experimental design is given in Figure 1.

Preparation of Leaf and Flower Extracts
A 100 mg fresh weight (FW) portion of S. ebulus leaves or flowers was homogenized in a mortar with 1 mL of 100% HPLC-grade methanol for phenylpropanoid extraction, while a 50 mg FW portion of leaf or flower tissues was mixed in HPLC water for amino acid extraction.Samples were then incubated overnight in the dark at 4 °C [35].Extracts were centrifuged for 20 min at 16,000× g at 4 °C, and the respective supernatants were filtered through 0.2 µm Ministart SRT 15 filters (Sigma-Aldrich, Milan, Italy) and preserved in test tubes at −20 °C until chromatographic analyses.Both crude extracts were also tested in entomological bioassays against mosquitoes.

Preparation of Leaf and Flower Extracts
A 100 mg fresh weight (FW) portion of S. ebulus leaves or flowers was homogenized in a mortar with 1 mL of 100% HPLC-grade methanol for phenylpropanoid extraction, while a 50 mg FW portion of leaf or flower tissues was mixed in HPLC water for amino acid extraction.Samples were then incubated overnight in the dark at 4 • C [35].Extracts were centrifuged for 20 min at 16,000× g at 4 • C, and the respective supernatants were filtered through 0.2 µm Ministart SRT 15 filters (Sigma-Aldrich, Milan, Italy) and preserved in test tubes at −20 • C until chromatographic analyses.Both crude extracts were also tested in entomological bioassays against mosquitoes.
The amino acid contents were analyzed by the same UHPLC system above reported and equipped with an Agilent column (Zorbax Eclipse AAA column, 5 µm particle size, 4.6 mm internal diameter × 150 mm length; Agilent, Milan, Italy) kept at 40 • C. A precolumn derivatization was performed by neutralizing samples in 0.4 M borate buffer (pH 10.2) to ensure that the amino terminus of each amino acid was neutralized.Primary amines were then reacted with phthalaldehyde and secondary amines (such as proline) were reacted with 9-fluorenylmethylchloroformate.The analytical conditions for the UHPLC determination were as follows: 100% solvent A (demineralized water 40 mM sodium phosphate dibasic buffer (pH 7.8)) for the first 18 min followed by a 1 min linear gradient to 57% solvent B (acetonitrile:methanol:water, 45:45:10 v/v), progressively set to reach 100% solvent B in 4 min, followed by a 5 min linear gradient to 100% solvent A. The flow rate was 2 mL min −1 .Primary amino acids were detected with a fluorescence detector (FLD-3400 RS; Thermo Scientific) at 340 and 450 nm (excitation and emission fluorescence), whereas secondary amino acids were detected with the UV detector above reported at 262 nm [37].The standard curves were obtained by plotting increasing concentrations of standard water solutions as a function of peak area in UHPLC chromatograms.Alanine, arginine, aspartic acid, glycine, glutamic acid, glutamine, histidine, isoleucine, leucine, phenylalanine, serine, threonine, and valine were determined and quantified in each extract using the software reported above.Measurements were performed on three different extracts belonging to three biological replicates; two instrumental replicates were carried out for each extract.

Collection and Rearing of Mosquito Eggs and Larvae
Over the Summer and early Autumn of 2021, we collected Ae. albopictus eggs by placing ovitraps consisting of black pots provided with four brown masonite strips (ovistrips) in the garden of the entomology laboratory at the Department of Agriculture, Food and Environment (DAFE) of the University of Pisa (Italy), as seen in Müller et al. [38].The ovistrips were picked up and replaced every other day, and eggs were left to hatch in a plastic basin (35 × 27 × 13 cm) filled with aged tap water under laboratory conditions (25 ± 1 • C, 45 ± 5% RH, and natural photoperiod).Tap water was aged for 24 h to dissipate the chlorine.Ae. albopictus larvae were then reared using dry cat food as nourishment.At the same time, we collected Cx. pipiens egg rafts from concrete tanks (80 × 60 × 45 cm) placed in the same garden of the DAFE and let them hatch in a separate plastic basin filled with aged tap water and provided with dry cat food under the same laboratory conditions.The confirmation of the identification of the two mosquito species was performed on larvae thanks to the pictorial keys provided by Andreadis et al. [39].The fourth-instar larvae of the two species, both obtained from the eggs collected outdoors, were then employed in the larvicidal tests.

Toxicity Tests on Aedes albopictus and Culex pipiens Larvae
The larvicidal activity of the leaf and flower S. ebulus extracts and the selected phenolic and amino acid compounds was evaluated on Ae. albopictus and Cx.pipiens following the specific 2005 WHO protocol [40] with minor modifications.
Crude extracts of flowers and leaves at increasing concentrations ranging from 2.0 to 4.0 mg mL −1 were diluted in aged tap water.Likewise, single phenolic compounds at increasing concentrations ranging from 1.0 to 5.0 mg mL −1 and single amino acids ranging from 0.50 to 2.5 mg mL −1 were diluted in aged tap water.All the toxicity tests were preceded by preliminary assessments to select the most suitable concentrations to obtain mortality values >0% and <99%.Groups of ten newly emerged fourth-instar larvae (0-24 h old) of both species were separately put in beakers containing 250 mL of solution of the S. ebulus extracts or singular compounds at the different concentrations indicated.As a negative control for vegetal extracts and phenylpropanoids, ten larvae were put in 250 mL of a solution of aged tap water and methanol at the concentration of 50 µL mL −1 (same quantity of methanol in the extracts and phenylpropanoid solutions at the highest concentration tested).For amino acids, controls were performed in 250 mL of aged tap water.For each treatment, control, and mosquito species, we performed four replicates.During the test, no food was given to the larvae according to Conti et al. [41].Larval mortality was recorded after the 24 h of permanence in the treatments.

Acetylcholinesterase Extraction and Inhibition Effect on Aedes albopictus and Culex pipiens Larvae
Since one of the most frequently reported modes of action on insects exerted by plant compounds, especially phenols, is the inhibition of AChE, we extracted this enzyme and evaluated its inhibition according to Bedini et al. [42,43] with minor modifications.We exclusively tested the effect of S. ebulus leaf and flower extracts on Ae. albopictus and Cx.pipiens larvae.An aliquot consisting of 300 mg of fourth-instar larvae of both mosquito species was individually homogenized in 4 mL of a buffer (10 mM Tris-HCl, pH 8.0) containing 0.5% (v/v) Triton X-100 and 20 mM NaCl.The homogenate was centrifuged at 17,000× g at 4 • C for 15 min, and the supernatant containing the AChE was filtered through glass wool to remove any excess lipids.The total protein content was quantified by the Protein Assay Kit II (Bio-Rad Laboratories, Inc., Hercules, CA, USA), and the enzymatic extract was used for the following assay.
Inhibition of AChE was determined by the classical colorimetric method of Ellman et al. [44], using acetylthiocholine (ACh) as substrate.The protein content of the AChE extract was diluted to 0.1 mg mL −1 , and the reaction mixture consisted of 500 µL of diluted AChE extract (which contained 0.05 mg of protein) and 50 µL of leaf or flower extracts for each concentration (2, 5, 25, 50, 100, 125, 250, and 500 µL mL −1 ) dissolved in 100% (v/v) methanol.Pure methanol was added to reach the final volume of 1 mL in the cuvette.Negative controls were prepared by adding methanol at the same concentrations but without the extracts.The tube was set in an incubator at 25 • C for 5 min before adding 100 µL of 0.01 M5, 5 ′ -dithiobis-(2-nitrobenzoic acid) (DTNB; dissolved in phosphate buffer pH 7.0) and 2.4 mL of phosphate buffer (pH 8.0).The mixture was gently stirred and incubated for 10 min at 25 • C before adding 40 µL of 75 mM ACh (dissolved in 0.1 M phosphate buffer pH 8.0) and then incubated again for 20 min at 25 • C.
The AChE activity was measured using an Ultrospec2100 Pro spectrophotometer (GE Healthcare Ltd., Amersham, UK) at 25 • C, by measuring the increase in absorbance at 412 nm.The inhibition percentage of AChE activity was calculated as follows: where SAT is the specific activity of the enzyme in the treated group and SAC is the specific activity of the enzyme in the control group.
The residual percentage of AChE activity was calculated as: Residual percentage % = (SAT/SAC) × 100 For each S. ebulus extract, concentration, and mosquito species, we performed three replicates.

Oviposition Deterrence towards Aedes albopictus in the Open Field
As the reproductive ethology of Cx. pipiens is completely different from that of Ae. albopictus, oviposition deterrence tests were only carried out on the latter species.Actually, Cx. pipiens lays its eggs in large natural bodies of water where it is not possible to test the extracts, whereas Ae. albopictus oviposits in small containers, such as the ovitraps previously described.Therefore, the oviposition deterrence exerted by the S. ebulus leaf and flower extracts was evaluated only on Ae. albopictus gravid females in the open field, according to the methodology described by Benelli et al. [45].The trials were carried out in the garden of the entomology laboratory at the DAFE from June to August 2022.The S. ebulus extracts were separately tested at the concentration of 2.0 mg mL −1 in aged tap water.Such concentration was chosen to be slightly below the LC 50 for both extracts.For each treatment, a black pot was filled with 500 mL of the solution; as a negative control, we used 500 mL of aged tap water.The three pots (two treatments, meaning the two extracts, and one control) were arranged in lines and separated by 50 cm among each other and 80 cm away from the other groups of pots.The position of the pots was alternated among the five replicates to avoid oviposition bias due to positional effects [45].In each pot belonging to the treated or control group, we placed one brown masonite strip (200 × 25 mm) (ovistrip) to allow Ae. albopictus females to lay eggs on.The number of eggs on the ovistrips was counted five times (i.e., after 1, 2, 3, 4, and 7 days) under a stereomicroscope (Leica EZ4, Leica Biosystems Italia, Buccinasco, Italy).All the ovistrips were collected and replaced in correspondence with each egg count.The data were analysed as Oviposition Activity Index (OAI), using the following formula by Kramer and Mulla [46]: where NT is the total number of eggs in the treated pots and NC is the total number of eggs in the control pots.Positive OAI values indicate that more eggs were laid in the treated pots than in the control ones, so the tested extract was attractive.Conversely, negative OAI values indicate that more eggs were laid in the control pots than in the treated ones, so the tested extract was repellent [46].

Data Analyses
The effects of vegetal tissue (leaf vs. flower) on biochemical parameters (i.e., phenylpropanoids and amino acids) were analysed by the Student's t-test.
The median lethal concentration (LC 50 ) of the S. ebulus extracts and phenolic compounds against Ae.albopictus and Cx.pipiens larvae was calculated by Log-probit regression [47].The fitness of the probit model (PROBIT(p) = Intercept + BX; where PROBIT(p) is the cumulative probability estimates, B is the slope of the model, and X is the extract concentration transformed using the base 10 logarithm (covariate)) was tested through the Pearson Goodness-of-Fit Test.A heterogeneity factor was used in the calculation of confidence limits when the significance level was less than 0.150.Differences between LC 50 values were assessed by Relative Median Potency (RMP) estimates, and they were considered significant if the RMP 95% confidence interval did not include 1. Differences between mosquito species susceptibility and among S. ebulus extracts and phenolic compounds toxicity were tested by one-way between-group univariate analysis of covariance (ANCOVA), with the chemical compound (extract or phenol) as a fixed factor and the concentration applied as a covariate to control its effects in the model.The mean response for each factor (chemical compound), adjusted for the concentration, was reported as estimated marginal (EM) means, and significant differences among them were determined by post-hoc comparisons using Bonferroni corrections for multiple comparisons.Statistical analyses were performed by the SPSS 22.0 software (IBM SPSS Statistics, Armonk, North Castle, NY, USA).
Data of AChE activities were arcsine transformed before analyses (after checking with the Shapiro-Wilk test the normal distribution of data) and then subjected to one-way analysis of variance (ANOVA).Significant differences between extract concentrations (within each species and plant organ) were determined by Fisher's least significant difference (LSD) post-hoc test (p ≤ 0.05).ANOVA statistical analyses were performed using GraphPad (GraphPad, La Jolla, CA, USA).
Oviposition Activity Index values ≥ 0.3 were considered attractive, and values ≤ −0.3 were repellent according to Kramer and Mulla [46].

Chemical Composition
Twelve phenylpropanoids were detected in methanol extracts from leaf and flower materials: seven phenolic compounds (four hydroxycinnamic acids and three hydroxybenzoic acids), four flavonoids (two flavones, one flavonol glycoside, and one flavonol), and one catechin (Table 1).Overall, hydroxycinnamic acids represented the most abundant chemical class of phenylpropanoids in leaf and flower materials (in particular, sinapic acid exhibited the highest amount in both organs), followed by hydroxybenzoic acids (in particular, dihydroxybenzoic acid exhibited the highest amounts in leaf, whereas gallic acid was the most abundant in flower material) and flavonol (i.e., kaempferol in both organs).Conversely, flavones (apigenin and luteolin), flavonol glycoside (rutin), and catechin were far less represented (in the flower material).Fourteen amino acids were detected in water extracts from leaf and flower materials: eleven nonaromatic and three aromatic amino acids (Table 2).Among the eleven nonaromatic amino acids identified, glutamic acid and valine exhibited the highest amounts in leaf and flower extracts, respectively.Conversely, aromatic amino acids (phenylalanine, tyrosine, and serine) were far less represented (in particular, phenylalanine and tyrosine were detected only in the flower material).From the preliminary screening on all detected phenylpropanoids (see Table 1), only two hydroxycinnamic acids (chlorogenic and rosmarinic) and two hydroxybenzoic acids (gallic and hydroxybenzoic) were selected to be singularly tested on the mosquito species.Since the preliminary tests on amino acids were unclear, we continued our investigation on five nonaromatic (arginine, aspartate, glutamic acid, histidine, and threonine) and one aromatic (serine) amino acids.Such amino acids were selected because no significant differences were observed in terms of chemical abundance in leaf and flower material (see Table 2).

Larvicidal Activity of Sambucus ebulus Leaf and Flower Extracts and Their Phenolic Compounds
From our screening, the leaf and flower extracts were found to have a toxic effect on the two mosquito larvae after 24 h.According to ANCOVA outputs, the larvicidal activity was dependent on the mosquito species (F 1,46 = 17.177; p < 0.001) and on the extract concentration (F 1,46 = 191.192;p < 0.001) but not on the plant organ (F 1,46 = 0.028; p = 0.868).Regarding the leaf extract, the most susceptible species to it was Ae. albopictus with an LC 50 value of 2.55 mg mL −1 , whereas the LC 50 value for Cx.pipiens was 3.18 mg mL −1 (Table 3).The RMP analysis showed that the difference in the susceptibility between the two species was significant (Ae.albopictus vs. Cx.pipiens RMP = 1.244;CI: 1.123-1.426).Conversely, Cx. pipiens larvae were the more susceptible to the extract from S. ebulus flower, with an LC 50 value of 2.77 mg mL −1 (Table 3).The RMP analysis showed that the difference in the susceptibility between the two species was significant (Ae.albopictus vs. Cx.pipiens RMP = 1.069;CI: 0.814-1.468).
The selected phenylpropanoids from S. ebulus showed toxic activity against the mosquito larvae, with LC 50 values ranging from 2.37 to 3.61 mg mL −1 for Ae.albopictus (Table 4) and from 3.55 to 3.91 mg mL −1 for Cx.pipiens (Table 4).Anyhow, both for Ae.albopictus and Cx.pipiens larvae, the RMP analyses indicated no significant differences among the phenolic compounds' toxicity.In accordance with the probit analyses, the ANCOVA indicated no statistically significant differences between species (F 1,87 = 1.623, p = 0.206) nor among the selected phenylpropanoids of S. ebulus (F 3,87 = 1.191, p = 0.318) but a significant interaction between species and compounds (F 2,32 = 13.559,p < 0.001).In detail, there was a significant effect of the concentration of the phenolic compounds on Cx. pipiens larvae mortality (F 2,32 = 9.666, p < 0.001) and, for Ae.albopictus, a significant effect of both concentration and the phenol on larval mortality (F 1,43 = 211.824,p < 0.001 and F 3,43 = 4.338, p = 0.009, respectively).
Conversely, all tested amino acids were unable to exert toxicity on the larvae of the two mosquito species at the applied concentrations (mortality was 4.7% only at the highest concentration tested of glutamic acid, namely 2.5 mg mL −1 , and null for the others).We decided not to test any further concentrations, as the amino acids' toxicity was not measurable in correspondence with values that almost represented the LC 50 for the other compounds and extracts involved in the study.

Acetylcholinesterase Inhibition in Aedes albopictus and Culex pipiens Larvae
The S. ebulus leaf and flower extracts inhibited the in vitro activities of AChE isolated from both Ae.albopictus and Cx.pipiens larvae (Figure 2).Overall, the leaf extract was more effective in AChE inhibition when compared to the flower one, and the effect was consistent for both the mosquito species under investigation.In particular, the residual AChE activities declined starting from 25 µL mL −1 (for Cx. pipiens) and 50 µL mL −1 (for Ae. albopictus) and then paralleled the severity of the treatment.With the flower extract, the inhibitory effect was milder, as only the two highest doses (250 and 500 µL mL −1 ) resulted in dramatic losses of AChE catalytic efficiency tested in vitro.

Acetylcholinesterase Inhibition in Aedes albopictus and Culex pipiens Larvae
The S. ebulus leaf and flower extracts inhibited the in vitro activities of AChE isol from both Ae.albopictus and Cx.pipiens larvae (Figure 2).Overall, the leaf extract was m effective in AChE inhibition when compared to the flower one, and the effect was sistent for both the mosquito species under investigation.In particular, the residual A activities declined starting from 25 µL mL −1 (for Cx. pipiens) and 50 µL mL −1 (for Ae bopictus) and then paralleled the severity of the treatment.With the flower extract, inhibitory effect was milder, as only the two highest doses (250 and 500 µL mL −1 ) resu in dramatic losses of AChE catalytic efficiency tested in vitro.

Repellency towards Aedes albopictus Gravid Females in the Open Field
From our screening in the open field, the leaf extract deterred the oviposition by albopictus starting from the third day after exposure to the treatments.On the contra slightly attractive effect was observed for the flower extract, apart from the fourth

Repellency towards Aedes albopictus Gravid Females in the Open Field
From our screening in the open field, the leaf extract deterred the oviposition by Ae. albopictus starting from the third day after exposure to the treatments.On the contrary, a slightly attractive effect was observed for the flower extract, apart from the fourth day, when the observed effect was a reduction in oviposition.However, the fluctuation of this OAI value around the average (−0.32 ± 0.25) indicates that, in a large proportion of cases, the activity was not significant (Table 5).

Discussion
Many phytochemical compounds were isolated and identified in different organs of S. ebulus, such as phenylpropanoids (i.e., caffeic acid derivatives and flavonoids), amino acids (i.e., ebulitins), steroids, and tannins [12].The main constituents with therapeutic properties of this plant are the phenolic compounds, found in great numbers in S. ebulus leaves and flowers, which are associated with organoleptic, nutritional, and antioxidant properties [13].Some of them are common in other medicinal plants too (e.g., Hypericum perforatum L.-Hypericaceae, Melissa officinalis L.-Lamiaceae, Salvia officinalis L.-Lamiaceae, as seen in Pellegrini et al. [35], Döring et al. [48], and Marchica et al. [36]) and are responsible for the antioxidant effects.In addition, ebulitin, ebulin 1, flavonoid, anthocyanin, and other components were isolated from S. ebulus and identified as other active ingredients with biological and pharmacological activities [12,14].In our work, we identified twelve phenylpropanoids through UHPLC, and all have been already reported in S. ebulus leaf extracts through similar experimental methods and often detected also in dwarf elder roots and fruits [49,50].Among them, neochlorogenic acid, rosmarinic acid, gallic acid, kampferol, and apigenin were also recorded in dwarf elder flowers extracts [51].To the best of our knowledge, although the phytochemical composition of S. ebulus fruits is well characterized with a detailed list of the amino acidic component [12], the general amino acid profile of S. ebulus leaves and flowers has not been deeply investigated.However, from the accurate description in terms of molecular and biological properties of ebulitins, a specific class of proteins extracted from dwarf elder leaves [52], we found that their structure made of sixteen amino acids matches the leaf profile of S. ebulus crude extract (in water) resulting from the analyses carried out in this work for fourteen (only cysteine and methionine do not coincide).
As stated before, this is the first attempt to test the dwarf elder in the entomological field, despite its folkloristic use against external parasites in livestock [15,16] as an insect repellent [17].To the best of our knowledge, there are no studies about the application of S. ebulus, nor even plants belonging to the same genus or family (Adoxaceae), to control insect Once penetrated, the bioactive compounds can impact the nervous system and alter the functioning of several enzymes by increasing the ATPase activity and inhibiting the cytochrome P-450 monooxygenase, carboxylesterase, and AChE [62].AChE is the enzyme catalysing the breakdown of the neurotransmitter acetylcholine and is found in neuroneuronal and neuromuscular junctions in insects and mammals, but insect AChE differs from mammal AChE by a cysteine residue making it a crucial insect-selective target [63].In the case here reported, using the colorimetric method of Ellman et al. [44], especially the S. ebulus leaf extract significantly inhibited the in vitro activity of the AChE isolated from both Cx.pipiens and Ae.albopictus individuals from, respectively, 25 and 50 µL mL −1 .Following a similar protocol, Demouche et al. [56] indicated a percentage of AChE inhibitory activity corresponding to 30.98 ± 2.97% in Cx. pipiens fourth-instar larvae into contact with a methanolic extract of dried aerial parts of Cotula cinerea Delile (Asteraceae) at 0.90 mg mL −1 .Moreover, through a semi-microtechnique, El Hadidy et al. [62] assessed that the AChE of Cx. pipiens third-instar larvae was reduced by, respectively, 57.86, 40.97, and 15.95% when treated with hexane extracts from the dried flowers, leaves, and stems of Ageratum houstonianum Mill.(Asteraceae) at concentrations of 259.79, 266.85, and 306.86 ppm.
At the alimentary canal level, some extracts can damage the digestive cells and degrade the microvilli and peritrophic membrane, causing the release of the gut content, disruption in the absorption of nutrients, and imbalanced homeostasis.Such histopathological alterations were shown in Cx. pipiens third-instar larvae treated with a Lepidium sativum L. (Brassicaceae) ethyl acetate extract [55].However, further research is needed to verify whether this is an additional mode of action that S. ebulus extracts can have on the two mosquito species involved in the study here reported.
In addition to the acute toxicity and physiological and morphological alterations in larvae, some vegetal extracts can similarly affect pupae [53,56] and cause weakness and fly inability in the adults emerged from specimens that survived treatments [54].
Some authors used organic solvents other than methanol to extract the bioactive compounds from different plants or dried powders obtained from vegetal tissues as repellents or mosquitocidals.It would be interesting to investigate the physiological and morphological changes in mosquitoes treated with similar S. ebulus products to better understand their effectiveness and possible mode of action.

Conclusions
The control of mosquito-borne diseases vectors is of unquestionable importance.Considering that their eradication is not realistically possible, limiting their presence and, consequently, the transmission of bacteria, parasites, and viruses, should be the main goal.
IVM of Ae. albopictus and Cx.pipiens on several fronts, involving not only chemical insecticides in emergency situations but also biological control agents or botanicals, could be a promising strategy.Overall, the S. ebulus leaf and flower extracts and their selected phenolic compounds proved to produce a toxic action on Ae. albopictus and Cx.pipiens larvae.Especially in our case, the crude dwarf elder extracts were roughly as toxic as their main phenolic compounds; therefore, the supplementary steps for their isolation could be avoided.
In conclusion, in addition to being a valuable way to exploit wild plants, the application of vegetal extracts is more affordable, ecological, and safer compared to chemical insecticides and could effectively help in the IVM of health-threatening mosquito populations.However, in order for vegetal extracts to be recommended and used by official bodies (ISS), the challenge has to be taken up by the industry, which will have to formulate and dose them in the most appropriate way.

Figure 1 .
Figure 1.Diagram of the experimental design, starting from the extraction of Sambucus ebulus leaves and flowers and continuing with the chemical determination and identification of the phenylpropanoids and amino acids contained and entomological bioassays (larval toxicity, acetylcholinesterase inhibition effect, and oviposition deterrence).

Figure 1 .
Figure 1.Diagram of the experimental design, starting from the extraction of Sambucus ebulus leaves and flowers and continuing with the chemical determination and identification of the phenylpropanoids and amino acids contained and entomological bioassays (larval toxicity, acetylcholinesterase inhibition effect, and oviposition deterrence).

Figure 2 .
Figure 2. In vitro residual percentage of AChE activity on Aedes albopictus and Culex pipiens afte application of the leaf and flower extracts of Sambucus ebulus.Data are given as means (n = standard error.Different letters are significantly different after one-way ANOVA followe Fisher's LSD post-hoc test (p ≤ 0.05).

Figure 2 .
Figure 2. In vitro residual percentage of AChE activity on Aedes albopictus and Culex pipiens after the application of the leaf and flower extracts of Sambucus ebulus.Data are given as means (n = 3) ± standard error.Different letters are significantly different after one-way ANOVA followed by Fisher's LSD post-hoc test (p ≤ 0.05).

Table 2 .
Nonaromatic and aromatic amino acids (mg g −1 fresh weight) in Sambucus ebulus leaves and flowers.Data are shown as means ± standard errors (n = 3 biological replicates for each tissue extract).For each compound, significant differences between the two plant organs are for ** p ≤ 0.01; * p ≤ 0.05; ns > 0.05.nd: not detected.

Table 4 .
Toxicity of the phenolic compounds extracted from Sambucus ebulus against Aedes albopictus and Culex pipiens larvae after 24 h.

Table 5 .
[46]ct of Sambucus ebulus leaf and flower extracts against the oviposition of the mosquito Aedes albopictus over a week.Extracts concentration: 2.0 mg mL −1 .Data are given as means ± standard error (n = 5).OAI, oviposition activity index.OAI values ≥ 0.3 indicate that extracts were attractive; OAI values ≤−0.3 indicate that extracts were repellent according to Kramer and Mulla[46](in bold).